Your search keyword '"Tiesman JP"' showing total 2 results

1. Spike-in genomic DNA for validating performance of metagenomics workflows.

Author

Venkataraman A, Parlov M, Hu P, Schnell D, Wei X, and Tiesman JP

Subjects

Bacteria isolation & purification, DNA, Bacterial isolation & purification, Gene Library, Genome, Bacterial, Humans, Rhodopseudomonas genetics, Rhodopseudomonas isolation & purification, Bacteria genetics, DNA, Bacterial genetics, High-Throughput Nucleotide Sequencing methods, Metagenomics methods, Microbiota, Workflow

Abstract

Shotgun metagenomics is a powerful platform to characterize human microbiomes. However, to translate such survey data into consumer-relevant products or services, it is critical to have a robust metagenomics workflow. We present a tool - spike-in DNA - to assess performance of metagenomics workflows. The spike-in is DNA from two organisms - Alivibrio fischeri and Rhodopseudomonas palustris, in a ratio of 4:1 added to samples before DNA extraction. With a valid workflow, the output ratio of relative abundances of these organisms should be close to 4. This expectation was tested in samples of varying diversities (n = 110), and the mean ratio was 4.73 (99% CI [4.0, 5.24]). We anticipate this tool to be a relevant community resource for assessing the quality of shotgun metagenomics workflows and thereby enable robust characterization of microbiomes.

Published

2018

2. Analysis of Affymetrix GeneChip data using amplified RNA.

Author

Cope L, Hartman SM, Göhlmann HW, Tiesman JP, and Irizarry RA

Subjects

Algorithms, DNA, Complementary genetics, DNA-Directed RNA Polymerases, Microdissection, Nucleic Acid Hybridization, RNA genetics, Transcription, Genetic, Viral Proteins, Nucleic Acid Amplification Techniques methods, Oligonucleotide Array Sequence Analysis methods, RNA analysis

Abstract

When small biological samples are collected by microdissection or other methods, amplification techniques are required to provide sufficient target for hybridization to expression arrays. One such technique is to perform two successive rounds of T7-based in vitro transcription. However the use of random primers, required to regenerate cDNA from the first round of transcription, results in shortened copies of cDNA from which the 5' end is missing. In this paper we describe an experiment designed to compare the quality of data obtained from labeling small RNA samples using the Affymetrix Two-Cycle Eukaryotic. Target Labeling procedure to that of data obtained using the One-Cycle Eukaryotic Target Labeling protocol. We utilized different preprocessing algorithms to compare the data generated using both labeling methods and present a new algorithm that improves upon existing ones in this setting.

Published

2006